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A practical guide to the synthesis and use of membrane-permeant acetoxymethyl esters of caged inositol polyphosphates

Subjects

Abstract

This protocol describes a method for efficient chemical synthesis of an analog of inositol-1,4,5-trisphosphate (IP3) hexakis acetoxymethyl ester having an ortho-nitroveratryl photochemical caging group on the 6-hydroxyl position. The six esters render the probe membrane permeant, such that it can be loaded into intact living cells in vitro or in vivo. Inside cells, the caged IP3 is inert until activated by two-photon excitation at 720 nm. The photoliberated signaling molecule can mobilize release of Ca2+ from intracellular stores on the endoplasmic reticulum. When co-loaded with the fluorescent Ca2+ indicator rhod-2, one laser can be used for stimulating and monitoring intracellular Ca2+ signaling with single-cell resolution. This protocol has chemistry and biology sections; the former describes the organic synthesis of the caged IP3, which requires 12 d, and the latter an application to a day-long study of astrocyte-regulated neuronal function in living brain slices acutely isolated from rats. As Ca2+ is the single most important intracellular second messenger and the IP3-Ca2+ signaling cascade is used by many cells to produce increases in Ca2+ concentration, this method should be widely applicable for the study of a variety of physiological processes in intact biological systems.

Acknowledgements

This work was supported by a grant from US NIH (GM53395) to G.C.R.E.-D. B.A.M. is a Canada Research Chairperson, and the acute slice work was supported by an operating grant from the Canadian Institutes of Health Research. G.R.J.G. is supported by the Alberta Heritage Foundation for Medical Research, the Michael Smith Foundation for Health Research and the Natural Sciences and Engineering Council of Canada.

Author information

Affiliations

Department of Neuroscience, Mount Sinai School of Medicine, New York, New York, USA.

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Contributions

S.K. prepared the caged compound. S.K. and G.C.R.E.-D. characterized the caged compound. G.C.R.E.-D. analyzed the NMR spectra. G.R.J.G. performed the cellular uncaging experiment. G.C.R.E.-D. wrote the paper with help from B.A.M. and G.R.J.G.